Direct reprogramming of fibroblasts into skeletal muscle progenitor cells by transcription factors enriched in undifferentiated subpopulation of satellite cells

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作者
Naoki Ito
Isao Kii
Noriaki Shimizu
Hirotoshi Tanaka
Shin’ichi Takeda
机构
[1] National Institute of Neuroscience,Department of Molecular Therapy
[2] National Center of Neurology and Psychiatry,Department of Rheumatology and Allergy
[3] IMSUT Hospital,Pathophysiological and Health Science Team, Imaging Application Group, Division of Bio
[4] The Institute of Medical Science,Function Dynamics Imaging
[5] The University of Tokyo,Division of Rheumatology, Center for Antibody and Vaccine Therapy, IMSUT Hospital
[6] Riken Center for Life Science Technologies,undefined
[7] The Institute of Medical Science,undefined
[8] The University of Tokyo,undefined
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Satellite cells comprise a functionally heterogeneous population of stem cells in skeletal muscle. Separation of an undifferentiated subpopulation and elucidation of its molecular background are necessary to identify the reprogramming factors to induce skeletal muscle progenitor cells. In this study, we found that intracellular esterase activity distinguishes a subpopulation of cultured satellite cells with high stemness using esterase-sensitive cell staining reagent, calcein-AM. Gene expression analysis of this subpopulation revealed that defined combinations of transcription factors (Pax3, Mef2b, and Pitx1 or Pax7, Mef2b, and Pitx1 in embryonic fibroblasts, and Pax7, Mef2b and MyoD in adult fibroblasts) reprogrammed fibroblasts into skeletal muscle progenitor cells. These reprogrammed cells formed Dystrophin-positive mature muscle fibers when transplanted into a mouse model of Duchenne muscular dystrophy. These results highlight the new marker for heterogenous population of cultured satellite cells, potential therapeutic approaches and cell sources for degenerative muscle diseases.
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